Abstract
In vitro selection coupled with directed evolution represents a powerful method for generating nucleic acids and proteins with desired functional properties. Creating high-quality libraries of random sequences is an important step in this process as it allows variants of individual molecules to be generated from a single-parent sequence. These libraries are then screened for individual molecules with interesting, and sometimes very rare, phenotypes. Here, we describe a general method to introduce random nucleotide mutations into a parent sequence that takes advantage of the polymerase chain reaction (PCR). This protocol reduces mutational bias often associated with error-prone PCR methods and allows the experimenter to control the degree of mutagenesis by controlling the number of gene-doubling events that occur in the PCR reaction. The error-prone PCR method described here was used to optimize a de novo evolved protein for improved folding stability, solubility, and ligand-binding affinity.
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References
Wilson DS, Szostak JW (1999) In vitro selection of functional nucleic acids. Annu Rev Biochem 68:611–647
Arnold FH, Georgiou G (2003) Directed enzyme evolution: screening and selection methods. Humana Press, New Jersey
Chaput JC, Woodbury NW, Stearns LA, Williams BAR (2008) Creating protein biocatalysts as tools for future industrial applications. Expert Opin Biol Ther 8:1087–1098
Arnold FH, Georgiou G (2003) Directed evolution library creation: methods and protocols. Humana Press, New Jersey
Leung DW, Chen E, Goeddel DV (1989) A method for random mutagenesis of a defined DNA segment using a modified polymerase chain reaction. Technique 1:11–15
Cadwell RC, Joyce GF (1992) Randomization of genes by PCR mutagenesis. PCR Methods Appl 2:28–33
Wilson DS, Keefe AD (2000) Random mutagenesis by PCR. Current protocols in molecular biology. Wiley, New Jersey
Smith MD, Rosenow MA, Wang M, Allen JP, Szostak JW, Chaput JC (2007) Structural insight into the evolution of a non-biological protein: importance of surface residues in protein fold optimization. PLoS ONE 2:e467
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© 2010 Humana Press
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McCullum, E.O., Williams, B.A.R., Zhang, J., Chaput, J.C. (2010). Random Mutagenesis by Error-Prone PCR. In: Braman, J. (eds) In Vitro Mutagenesis Protocols. Methods in Molecular Biology, vol 634. Humana Press, Totowa, NJ. https://doi.org/10.1007/978-1-60761-652-8_7
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DOI: https://doi.org/10.1007/978-1-60761-652-8_7
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Publisher Name: Humana Press, Totowa, NJ
Print ISBN: 978-1-60761-651-1
Online ISBN: 978-1-60761-652-8
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